An accurate, reliable, and universal qPCR method to identify homozygous single insert T-DNA with the example of transgenic rice
Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development o...
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| Published in | Frontiers in plant science Vol. 14; p. 1221790 |
|---|---|
| Main Authors | , , , , , , |
| Format | Journal Article |
| Language | English |
| Published |
Frontiers Media S.A
10.10.2023
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| Subjects | |
| Online Access | Get full text |
| ISSN | 1664-462X 1664-462X |
| DOI | 10.3389/fpls.2023.1221790 |
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| Abstract | Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development of multiple homozygous transgenic rice lines in the T
1
generation, with low copy number to single T-DNA insert for further analyses. Here, a well-established qPCR protocol, based on the
OsSBE4
reference gene and the
nos
terminator, was optimized in the transgenic Japonica rice cultivar Nipponbare, to distinguish homozygous single-insert plants with 100% accuracy. This method was successfully adapted to transgenic Indica rice plants carrying three different T-DNAs, without any modifications to quickly develop homozygous rice plants in the T
1
generation. The accuracy of this qPCR method when applied to transgenic Indica rice approached 100% in 12 putative transgenic lines. Moreover, this protocol also successfully detected homozygous single-locus T-DNA transgenic rice plants with two-transgene T-DNAs, a feature likely to become more popular in future transgenic research. The assay was developed utilizing universal primers targeting common sequence elements of gene cassettes (the
nos
terminator). This assay could therefore be applied to other transgenic plants carrying the
nos
terminator. All procedures described here use standardized qPCR reaction conditions and relatively inexpensive dyes, such as SYBR Green, thus the qPCR method could be cost-effective and suitable for lower budget laboratories that are involved in rice transgenic research. |
|---|---|
| AbstractList | Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development of multiple homozygous transgenic rice lines in the T
1
generation, with low copy number to single T-DNA insert for further analyses. Here, a well-established qPCR protocol, based on the
OsSBE4
reference gene and the
nos
terminator, was optimized in the transgenic Japonica rice cultivar Nipponbare, to distinguish homozygous single-insert plants with 100% accuracy. This method was successfully adapted to transgenic Indica rice plants carrying three different T-DNAs, without any modifications to quickly develop homozygous rice plants in the T
1
generation. The accuracy of this qPCR method when applied to transgenic Indica rice approached 100% in 12 putative transgenic lines. Moreover, this protocol also successfully detected homozygous single-locus T-DNA transgenic rice plants with two-transgene T-DNAs, a feature likely to become more popular in future transgenic research. The assay was developed utilizing universal primers targeting common sequence elements of gene cassettes (the
nos
terminator). This assay could therefore be applied to other transgenic plants carrying the
nos
terminator. All procedures described here use standardized qPCR reaction conditions and relatively inexpensive dyes, such as SYBR Green, thus the qPCR method could be cost-effective and suitable for lower budget laboratories that are involved in rice transgenic research. Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development of multiple homozygous transgenic rice lines in the T1 generation, with low copy number to single T-DNA insert for further analyses. Here, a well-established qPCR protocol, based on the OsSBE4 reference gene and the nos terminator, was optimized in the transgenic Japonica rice cultivar Nipponbare, to distinguish homozygous single-insert plants with 100% accuracy. This method was successfully adapted to transgenic Indica rice plants carrying three different T-DNAs, without any modifications to quickly develop homozygous rice plants in the T1 generation. The accuracy of this qPCR method when applied to transgenic Indica rice approached 100% in 12 putative transgenic lines. Moreover, this protocol also successfully detected homozygous single-locus T-DNA transgenic rice plants with two-transgene T-DNAs, a feature likely to become more popular in future transgenic research. The assay was developed utilizing universal primers targeting common sequence elements of gene cassettes (the nos terminator). This assay could therefore be applied to other transgenic plants carrying the nos terminator. All procedures described here use standardized qPCR reaction conditions and relatively inexpensive dyes, such as SYBR Green, thus the qPCR method could be cost-effective and suitable for lower budget laboratories that are involved in rice transgenic research. Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development of multiple homozygous transgenic rice lines in the T1 generation, with low copy number to single T-DNA insert for further analyses. Here, a well-established qPCR protocol, based on the OsSBE4 reference gene and the nos terminator, was optimized in the transgenic Japonica rice cultivar Nipponbare, to distinguish homozygous single-insert plants with 100% accuracy. This method was successfully adapted to transgenic Indica rice plants carrying three different T-DNAs, without any modifications to quickly develop homozygous rice plants in the T1 generation. The accuracy of this qPCR method when applied to transgenic Indica rice approached 100% in 12 putative transgenic lines. Moreover, this protocol also successfully detected homozygous single-locus T-DNA transgenic rice plants with two-transgene T-DNAs, a feature likely to become more popular in future transgenic research. The assay was developed utilizing universal primers targeting common sequence elements of gene cassettes (the nos terminator). This assay could therefore be applied to other transgenic plants carrying the nos terminator. All procedures described here use standardized qPCR reaction conditions and relatively inexpensive dyes, such as SYBR Green, thus the qPCR method could be cost-effective and suitable for lower budget laboratories that are involved in rice transgenic research.Early determination of transgenic plants that are homozygous for a single locus T-DNA insert is highly desirable in most fundamental and applied transgenic research. This study aimed to build on an accurate, rapid, and reliable quantitative real-time PCR (qPCR) method to fast-track the development of multiple homozygous transgenic rice lines in the T1 generation, with low copy number to single T-DNA insert for further analyses. Here, a well-established qPCR protocol, based on the OsSBE4 reference gene and the nos terminator, was optimized in the transgenic Japonica rice cultivar Nipponbare, to distinguish homozygous single-insert plants with 100% accuracy. This method was successfully adapted to transgenic Indica rice plants carrying three different T-DNAs, without any modifications to quickly develop homozygous rice plants in the T1 generation. The accuracy of this qPCR method when applied to transgenic Indica rice approached 100% in 12 putative transgenic lines. Moreover, this protocol also successfully detected homozygous single-locus T-DNA transgenic rice plants with two-transgene T-DNAs, a feature likely to become more popular in future transgenic research. The assay was developed utilizing universal primers targeting common sequence elements of gene cassettes (the nos terminator). This assay could therefore be applied to other transgenic plants carrying the nos terminator. All procedures described here use standardized qPCR reaction conditions and relatively inexpensive dyes, such as SYBR Green, thus the qPCR method could be cost-effective and suitable for lower budget laboratories that are involved in rice transgenic research. |
| Author | Jenkins, Colin L. D. Huynh, My-my Anderson, Peter A. Shavrukov, Yuri Tran, Hai Thanh Stangoulis, James C. R. Schramm, Carly |
| AuthorAffiliation | College of Science and Engineering, Flinders University , Adelaide, SA , Australia |
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| Author_xml | – sequence: 1 givenname: Hai Thanh surname: Tran fullname: Tran, Hai Thanh – sequence: 2 givenname: Carly surname: Schramm fullname: Schramm, Carly – sequence: 3 givenname: My-my surname: Huynh fullname: Huynh, My-my – sequence: 4 givenname: Yuri surname: Shavrukov fullname: Shavrukov, Yuri – sequence: 5 givenname: James C. R. surname: Stangoulis fullname: Stangoulis, James C. R. – sequence: 6 givenname: Colin L. D. surname: Jenkins fullname: Jenkins, Colin L. D. – sequence: 7 givenname: Peter A. surname: Anderson fullname: Anderson, Peter A. |
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| Cites_doi | 10.1093/nar/gkaa682 10.1007/s00299-004-0881-0 10.1111/j.1365-313X.2009.03942.x 10.1111/pce.12693 10.1186/1472-6750-4-14 10.1007/978-1-4939-0446-4_17 10.1007/BF02914056 10.1007/s11248-016-9982-0 10.1007/s12010-014-1322-3 10.21769/BioProtoc.4075 10.1186/1471-2229-13-71 10.1038/srep07358 10.1186/1472-6750-2-20 10.1023/B:MOLB.0000018767.64586.53 10.2144/01311rr04 10.1007/s00299-004-0859-y 10.1038/nature03895 10.1007/s00299-001-0432-x 10.1016/0307-4412(92)90202-W 10.1016/S0168-9452(02)00381-3 10.2478/s11658-011-0029-5 10.1007/978-1-4939-7337-8_15 10.1093/pcp/pce042 10.1111/tpj.13517 10.1021/jf803166p 10.3389/fpls.2018.01923 10.1016/s0022-2836(75)80083-0 10.1016/j.tig.2004.06.004 10.1006/meth.2001.1262 10.1007/BF02772725 10.1007/s002990100326 |
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| Copyright | Copyright © 2023 Tran, Schramm, Huynh, Shavrukov, Stangoulis, Jenkins and Anderson. Copyright © 2023 Tran, Schramm, Huynh, Shavrukov, Stangoulis, Jenkins and Anderson 2023 Tran, Schramm, Huynh, Shavrukov, Stangoulis, Jenkins and Anderson |
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| SubjectTerms | homozygous plant NOS terminator OsSBE4 reference gene Plant Science quantitative real-time PCR single T-DNA zygosity identification |
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| Title | An accurate, reliable, and universal qPCR method to identify homozygous single insert T-DNA with the example of transgenic rice |
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